New shuttle vectors for the introduction of cloned DNA in Desulfovibrio

New shuttle vectors for the introduction of cloned DNA in Desulfovibrio

The pBG1 replicon from the cryptic plasmid of Desulfovibrio desulfuricans G100A was inserted into pTZ18U derivatives to generate a new family of shuttle vectors. These plasmids are stable both in Escherichia coli and in Desulfovibrio, they present a large number of unique restriction sites, and colo...

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Veröffentlicht in:Plasmid 1998, Vol.39 (2), p.114-122
Hauptverfasser: Rousset, M, Casalot, L, Rapp-Giles, B J, Dermoun, Z, de Philip, P, Bélaich, J P, Wall, J D
Format: Artikel
Sprache:eng
Schlagworte:
Cloning, Molecular - methods
Conjugation, Genetic
Desulfovibrio - genetics
Electroporation
Escherichia coli - genetics
Genetic Vectors - genetics
Hydrogenase - genetics
Plasmids - genetics
Replicon - genetics
Transformation, Bacterial
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Zusammenfassung:The pBG1 replicon from the cryptic plasmid of Desulfovibrio desulfuricans G100A was inserted into pTZ18U derivatives to generate a new family of shuttle vectors. These plasmids are stable both in Escherichia coli and in Desulfovibrio, they present a large number of unique restriction sites, and colonies of recombinant clones can be identified by blue/white screening in E. coli. The pBMC, pBMK, and pBMS series carry the cat, npt, or strAB genes as selectable markers, respectively. The pBMC6, pBMK6, and pBMS6 plasmids can be introduced both in D. desulfuricans and in Desulfovibrio fructosovorans by electrotransformation, and the pBMC7, pBMK7, and pBMS7 plasmids contain additional mobilization functions which makes them suitable for conjugation.
ISSN:0147-619X
DOI:10.1006/plas.1997.1321